Quantification of viral DNA during HIV-1 infection: A review of relevant clinical uses and laboratory methods

E.K. Alidjinou, L. Bocket, D. Hober
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引用次数: 26

Abstract

Effective antiretroviral therapy usually leads to undetectable HIV-1 RNA in the plasma. However, the virus persists in some cells of infected patients as various DNA forms, both integrated and unintegrated. This reservoir represents the greatest challenge to the complete cure of HIV-1 infection and its characteristics highly impact the course of the disease. The quantification of HIV-1 DNA in blood samples constitutes currently the most practical approach to measure this residual infection. Real-time quantitative PCR (qPCR) is the most common method used for HIV-DNA quantification and many strategies have been developed to measure the different forms of HIV-1 DNA. In the literature, several “in-house” PCR methods have been used and there is a need for standardization to have comparable results. In addition, qPCR is limited for the precise quantification of low levels by background noise. Among new assays in development, digital PCR was shown to allow an accurate quantification of HIV-1 DNA. Total HIV-1 DNA is most commonly measured in clinical routine. The absolute quantification of proviruses and unintegrated forms is more often used for research purposes.

HIV-1感染期间病毒DNA的定量:相关临床应用和实验室方法的综述
有效的抗逆转录病毒治疗通常会导致血浆中检测不到HIV-1 RNA。然而,病毒以各种DNA形式存在于感染患者的某些细胞中,既有整合的,也有非整合的。这个病毒库是彻底治愈HIV-1感染的最大挑战,它的特点对疾病的进程有很大影响。血液样本中HIV-1 DNA的定量是目前测量这种残留感染最实用的方法。实时定量PCR (qPCR)是用于HIV-1 DNA定量的最常用方法,并且已经开发了许多策略来测量不同形式的HIV-1 DNA。在文献中,已经使用了几种“内部”PCR方法,需要标准化以获得可比较的结果。此外,qPCR对于低水平背景噪声的精确定量是有限的。在正在开发的新检测方法中,数字PCR被证明可以准确定量HIV-1 DNA。总HIV-1 DNA是临床常规中最常用的测量方法。原病毒和非整合形式的绝对定量更常用于研究目的。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Pathologie-biologie
Pathologie-biologie 医学-病理学
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审稿时长
6-12 weeks
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